[Construction of Saccharomyces cerevisiae cell factories for fermentation production of retinol].

Q3 Pharmacology, Toxicology and Pharmaceutics Zhongguo Zhongyao Zazhi Pub Date : 2024-08-01 DOI:10.19540/j.cnki.cjcmm.20240517.105
Wen-Hao Li, Ting-Ting Yang, Rui Li, Xiao-Chen Ma, Shi-Ru Jia, Xue-Li Zhang, Dong Wang, Zhu-Bo Dai
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Abstract

Retinol is one of the main active forms of vitamin A, crucial for the organism's growth, development, and maintenance of eye and skin functions. It is widely used in cosmetics, pharmaceuticals, and feed additives. Although animals lack a complete pathway for synthesizing vitamin A internally, they can obtain vitamin A directly through diet or convert β-carotene acquired from the diet. To boost the research on the biosynthesis of retinol, three different sources of alcohol dehydrogenase were firstly screened based on the β-carotene synthesis platform CAR*1. It was determined that ybbO from Escherichia coli exhibited the highest catalytic activity,with a conversion rate of 95. 6%. To further enhance the reaction rate and yield of retinol, protein fusion technology was employed to merge two adjacent enzymes, blh and ybbO, within the retinol synthesis module. The evaluation was conducted using the high-yield engineered strain CAR*3 of β-carotene. The optimal combination, blh-GGGS-ybbO, was obtained, with a 44. 9% increase in yield after fusion, reaching(111. 1± 3. 5) mg·L~(-1). Furthermore, through the introduction of human-derived retinol-binding protein(RBP4) and transthyretin(TTR), the process of hepatic cell secreting retinol was simulated in Saccharomyces cerevisiae, leading to an increased retinol yield of(158. 0±13. 1)mg·L~(-1). Finally, optimization strategies including overexpressing INO2 to enhance the reaction area for β-carotene synthesis, enhancing hemoglobin VHb expression to improve oxygen supply, and strengthening PDR3m expression to facilitate retinol transport were implemented. A two-stage fermentation process resulted in the successful elevation of retinol production to(2 320. 0±26. 0)mg·L~(-1) in the fermentation tank of 5 L, which provided a significant foundation for the industrial development of retinol.

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[构建用于发酵生产视黄醇的酿酒酵母细胞工厂]。
视黄醇是维生素 A 的主要活性形式之一,对生物体的生长、发育以及眼睛和皮肤功能的维持至关重要。它被广泛用于化妆品、药品和饲料添加剂。虽然动物体内缺乏合成维生素 A 的完整途径,但它们可以直接从食物中获取维生素 A,或将从食物中获取的 β-胡萝卜素转化为维生素 A。为了促进视黄醇生物合成的研究,首先以β-胡萝卜素合成平台CAR*1为基础,筛选了三种不同来源的醇脱氢酶。结果表明,来自大肠杆菌的 ybbO 具有最高的催化活性,转化率高达 95.6%。为了进一步提高视黄醇的反应速率和产量,研究人员采用了蛋白质融合技术,在视黄醇合成模块中合并了两个相邻的酶,即 blh 和 ybbO。评估使用了高产的β-胡萝卜素工程菌株CAR*3。获得的最佳组合是 blh-GGGS-ybbO,融合后产量提高了 44.9% ,达到(111. 1± 3. 5) mg-L~(-1)。此外,通过引入人源视黄醇结合蛋白(RBP4)和转甲状腺素(TTR),在酿酒酵母中模拟肝细胞分泌视黄醇的过程,使视黄醇产量增加到(158.最后,还实施了优化策略,包括过度表达 INO2 以增加合成 β-胡萝卜素的反应面积,增强血红蛋白 VHb 的表达以改善氧气供应,以及加强 PDR3m 的表达以促进视黄醇的转运。通过两级发酵工艺,在 5 L 发酵罐中成功将视黄醇产量提高到(2 320. 0±26. 0)mg-L~(-1),为视黄醇的工业化开发奠定了重要基础。
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来源期刊
Zhongguo Zhongyao Zazhi
Zhongguo Zhongyao Zazhi Pharmacology, Toxicology and Pharmaceutics-Pharmacology, Toxicology and Pharmaceutics (all)
CiteScore
1.50
自引率
0.00%
发文量
581
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